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Theoretical and experimental investigation of chaperone effects on soluble recombinant proteins in Escherichia coli: effect of free DnaK level on temperature-induced recombinant streptokinase production

机译:伴侣蛋白对大肠杆菌中可溶性重组蛋白影响的理论和实验研究:游离DnaK水平对温度诱导的重组链激酶产生的影响

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摘要

Modeling and analysis of genetic networks have become increasingly important in the investigation of cellular processes. The genetic networks involved in cellular stress response can have a critical effect on the productivity of recombinant proteins. In this work, it was found that the temperature-inducible expression system for the production of soluble recombinant streptokinase in Escherichia coli resulted in a lower productivity compared to the chemically-induced system. To investigate the effect of the induced cellular response due to temperature up-shift a model-based approach is adopted. The role played by the major molecular chaperone teams DnaK–DnaJ–GrpE and GroEL–GroES on the productivity of recombinant streptokinase was experimentally determined. Based on these investigations, a detailed mechanistic mathematical model was developed for the cellular response during the temperature-induced recombinant streptokinase production. The model simulations were found to have a good qualitative agreement with the experimental results. The mechanistic mathematical model was validated with the experiments conducted on a σ32 mutant strain. Detailed analysis of the parameter sensitivities of the model indicated that the level of free DnaK chaperone in the cell has the major effect on the productivity of recombinant streptokinase during temperature induction. Analysis of the model simulations also shows that down regulation or selective redirection of the heat shock proteins could be a better way of manipulating the cellular stress response than overexpression or deletion. In other words, manipulating the system properties resulting from the interaction of the components is better than manipulating the individual components. Although our results are specific to a recombinant protein (streptokinase) and the expression system (E. coli), we believe that such a systems-biological approach has several advantages over conventional experimental approaches and could be in principle extended to bigger genetic networks as well as other recombinant proteins and expression systems.Electronic supplementary materialThe online version of this article (doi:10.1007/s11693-009-9021-z) contains supplementary material, which is available to authorized users.
机译:在研究细胞过程中,遗传网络的建模和分析已变得越来越重要。涉及细胞应激反应的遗传网络可能对重组蛋白的生产率产生关键影响。在这项工作中,发现与化学诱导系统相比,在大肠杆菌中生产可溶性重组链激酶的温度诱导表达系统导致较低的生产率。为了研究由于温度上升引起的诱导细胞反应的影响,采用了基于模型的方法。实验确定了主要分子伴侣团队DnaK–DnaJ–GrpE和GroEL–GroES在重组链激酶活性上的作用。基于这些研究,针对温度诱导的重组链激酶生产过程中的细胞反应,建立了详细的力学数学模型。发现该模型仿真与实验结果具有良好的定性一致性。通过对σ 32 突变菌株的实验验证了该机理的数学模型。对模型参数敏感性的详细分析表明,细胞中游离DnaK分子伴侣的水平对温度诱导过程中重组链激酶的生产力有重要影响。对模型模拟的分析还表明,与过度表达或缺失相比,热激蛋白的下调或选择性重定向可能是操纵细胞应激反应的更好方法。换句话说,操纵由组件交互产生的系统属性比操纵单个组件要好。尽管我们的结果特定于重组蛋白(链激酶)和表达系统(大肠杆菌),但我们认为这种系统生物学方法相对于常规实验方法具有多个优势,并且原则上也可以扩展到更大的遗传网络电子补充材料本文的在线版本(doi:10.1007 / s11693-009-9021-z)包含补充材料,授权用户可以使用。

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